WO2016130616A1 - Bacteria over-expressing c-di-amp and therapeutic methods - Google Patents

Abstract

The present invention includes the discovery of a strain of Mycobacterium comprising an expression vector encoding a di-adenylate cyclase enzyme. The Mycobacterium is selected from the group consisting of Mycobacterium tuberculosis, Mycobacterium bovis, or a combination thereof and the preferred strain of Mycobacterium is BCG. The preferred expression vector is a mycobacterial expression vector including an hsp60 promoter and a DNA sequence of diadenylate cyclase (disA), or a functional part thereof. The strains of Mycobacterium are used in therapeutic applications including tuberculosis and cancer.?

Description

Bacteria Over-Expressing c-di-AMP and Therapeutic Methods

REFERENCE TO RELATED APPLICATIONS

[0001] This application claims the benefit of a US Provisional Application 62 114,610, filed February 11, 2015, which is hereby incorporated by reference for all purposes as if fully set forth herein.

STATEMENT OF GOVERNMENTAL INTEREST

[0002] This invention was made with government support under grant nos. A136973, A137856, A1097138 from the National Institutes of Health. The government has certain rights in the invention.

INCORPORATION-BY-REFERENCE

[0003] AH references, including publications, patent applications, and patents, cited herein are hereby incorporated by reference to the same extent as if each reference were individually and specifically indicated to be incorporated by reference and were set forth in its entirety herein.

BACKGROUND OF THE INVENTION

[0004] Nucleotides are indispensable components of all living cells, as they make up DNA and RNA, and serve as important energy sources. Nucleotides also have key roles in signaling In eukaryotic, bacterial and archaeal cells. In bacteria, signaling nucleotides such as cyclic AMP and guanosine tetra- or pentaphosphate ((p)ppGpp) have been classically linked to carbon metabolism and the stringent response, which is caused by nutrient limitation. However, it has become clear that signaling nucleotides contribute to the regulation of multiple different pathways; for example, in addition to its involvement in central carbon metabolism, cAMP is also involved in the regulation of both biofilm formation and virulence gene expression in many pathogenic bacteria. One of the latest signaling nucleotides- to be identified is cyclic di-AMP (c-di-AMP), which is the second cyclic dinuoleot.de shown to be produced by bacteria, after cyclic di-GMP (c-di-GMP). It has been suggested that c-di-AMP and c-di-GMP regulate veiy different processes. [0005] c-di-AMP is produced from two molecules of ATP by diadenylyl cyclase (DAC) enzymes and is degraded to pApA by phosphodiesterase (PDE) enzymes. The dinucleotide was initially discovered during a structural study on Thermotoga maritima.DNA integrity scanning protein (DisA), which is a homologue of Bacillus svbtilis DisA (formerly known as YacK), a bacterial DNA damage checkpoint protein that can delay sporulation in the event of DNA damage. The first report of c-di-AMP production by bacterial cells came in 2010, when the dinucleotide was identified as a molecule secreted into the cytosol of host cells by the intracellular bacterial pathogen Listeria monocytogenes. Since then, c-di-AMP has been detected in cellular extracts from Streptococcus pyogenes, B. subtills, Chlamydia trachomatis and Staphylococcus aureus, and a DisA-type c-di-AMP-synthesizing enzyme from

Mycobacterium tuberculosis has been characterized biochemically.

[0006] Although most of the mechanistic details still await molecular characterization, the regulation of cellular pathways by c-di-AMP presumably follows the same general principles as for the other signaling nucleotides. Environmental changes are sensed either directly or indirectly by the nucleotide-synmesizing or nucleotide-degrading enzymes, leading to a change in the cellular nucleotide concentration. At high concentrations, c-di- AMP is expected to bind to a specific set of receptor or target proteins and allosterically alter their function or the function of downstream effector proteins, thus controlling specific cellular pathways. Although many details of the c-di-AMP signaling network remain to be discovered, this nucleotide has been linked to the regulation of nitty acid synthesis in Mycobacterium smegmatis, to the growth of S. aureus in low-potassium conditions, to the sensing of DNA integrity in B. subtih^'ssnd to cell wall homeostasis in multiple species. 10007] The M. tuberculosis genome encodes a di-adenylate cyclase enzyme (disA, also called dacA; encoded by gene Rv3586 (also called MT3692) in the H37 v genome or MT3692 in the CDC 1551 genome) that synthesizes c-di-AMP from ATP or ADP4. Orthologs of disA exist in all mycobacterial genomes with the exception ofM. leprae. However, the role of c-di-AMP in M. tuberculosis physiology and mechanism of its interaction with the host immune system is poorly understood. However, the existing model for M. tuberculosis infection is that extracellular mycobacterial DNA is the only ligand for CSP activation within macrophages, which leads to increased autophagy and bacterial clearance in an ESX-1 secretion system-dependent manner, excluding any role for bacterial CDNs in CSP activation.

[0008] The mammalian innate immune system is composed of receptors that collectively serve as a pathogen sensor to monitor the extracellular, vacuolar, and cytosolic cellular compartments. Recognition of microbes within these distinct compartments leads to cellular responses that are commensurate with the microbial threat. Although both pathogenic and nonpathogenic microbes interact with extracellular and vacuolar compartments, infectious disease agents often mediate their pathogenesis by directly entering the cytosol or through delivery of virulence factors into the host cell cytosolic compartment Thus, the innate immune system may distinguish between pathogenic and nonpathogenic microbes by monitoring the cytosol.

[0009] Several distinct pathways of innate immunity are present in the host cell cytosol. One, termed the cytosolic surveillance pathway (CSP), detects bacterial, viral, and protozoan pathogens, leading to the activation of interferon regulatory factor 3 (IRF3) and nuclear factor kappa-light-chain-enhancer of activated B cells ( F-TCB), resulting in the induction of interferon-β (lFN-β) and co-regulated genes. Some ligands that activate this pathway are known, for example, viral and bacterial nucleic acids. However, the ligands and host receptors that lead to IFN-β production after exposure to nonviral microbes— including L. monocytogenes, M. tuberculosis, F. tul rensis, L. pneumophila, B. abortis, and T. cruzi— remain unknown. The mechanisms and role of c-di-AMP signaling in Mycobacterium tuberculosis infectionmust be identified and treatments mat prevent, alleviate, or cure tuberculosis must be developed.

[0010] Bacttle Cal ette Guerin (BCG) is the most widely used vaccination in the world. BCG is made of a live, weakened strain of Mycobacterium bovis, (a cousin of

Mycobacterium tuberculosis, the TB bacteria). It was developed in the I930's and it remains the only vaccination available against tuberculosis today. Despite its protection against active TB in children, BCG has failed to protect adults against TB infection and active disease development, especially in developing countries where the disease is endemic. Some of key reasons for failure of BCG is low immimogenicity and its inability to induce maturation of DC efficiently. Among various strategies that have been employed so far to improve the protective potential of BCG involve construction of rBCG, which could confer similar or higher protection along with induction of a better immunological memory than BCG. Most of the methodologies used to achieve greater immunogenicity involve (i) over-expression of promising immuno-dominant antigens either singularly or as fusion with other immunodominant antigens, (ii) over-expression and reintroduction of antigens lost during the attenuation process or (iii) over-expression of mammalian cytokines in BCG such as IL-2, IL- 12, IL-15, and GM-CSF. New methods of tuberculosis vaccination are needed to prevent the spread of disease.

[0011] fn addition, more than 60,000 new cases of bladder cancer are diagnosed each year in the United States accounting for approximately 13,000 deaths. BCG-based therapy is currently the most effective intravesical therapy for nonmuscle invasive bladder cancer (NMIBC) and it represents the only agent known to reduce the progression of invasive bladder cancer into muscle. It is widely accepted that an intact immune system is a prerequisite to a successful therapy. BCG-induced antitumor effects depend on a sequence of events involving a complex interplay of soluble and cellular immune mediators and a crosstalk between innate and adaptive immunity. Limitations of BCG therapy include recurrence of the disease after initiation of BCG therapy. Consequently, new BCG strains enhancing the prevention or cure, and minimizing the recurrence rate, of cancer in patients must be identified.

SUMMARY OF THE INVENTION

[0012] One embodiment of the invention is a pharmaceutical composition comprising a compound, salt, solvate, or stereoisomer of a synthetic c-di-AMP, and a pharmaceutically acceptable carrier. This pharmaceutical composition may include at least one or more other compounds enhancing immunogenicity such as mycobacterial DNA, IFN, or c-di-AMP and combinations thereof.

[0013] Another embodiment of the invention is a method of treating a bacterial infection in a subject comprising administering to the subject an effective amount of a compound, salt, solvate, or stereoisomer of synthetic c-di-AMP.

[0014] Another embodiment of the invention is a method of treating tuberculosis (TB) in a subject comprising administering an effective amount of a compound, salt, solvate, or stereoisomer of c-di-AMP. [0015] Another embodiment of the invention is the discovery of one or more strain(s) of Mycobacterium comprising an expression vector encoding a di-adenylate cyclase enzyme. - The Mycobacterium is preferably selected from the group consisting of Mycobacterium tuberculosis, Mycobacterium bovis, or a combination thereof, The preferred strain of Mycobacterium bovis is a Mycobacterium bovis bacille Calmette-Guerin strain ("BCG") that preferably over-expresses a diadenylate cyclase (disA) of M, tuberculosis ( v3586) from a mycobacterial expression vector (or plasmid). The most preferred strains are BCG- pSDhsp60.MT3692 (a BCG strain harboring the episomal plasmid pSDhsp60.MT3692), and BCG-pMH94Hyg.MT3692 (a BCG strain harboring the integrative plasmid

pMH94Hyg MT3692). Many strains of BCG maybe transformed with plasmids of the present invention, pSDhsp60.MT3692 and pMH94Hyg.MT3692 to form novel pharmaceutical compositions. The preferred mycobacterial expression vector includes an hsp60 promoter and a DNA sequence of diadenylate cyclase (disA), or a functional part thereof, wherein the expression of di-adenylate cyclase enzyme or a functional part thereof is regulated by the hsp60 promoter. The term "functional part thereof means a part of the diadenylate cyclase enzyme that maintains its enzymatic activity. The one or more strains of Mycobacterium described above are used in therapeutic applications including tuberculosis and cancer, specifically nonmuscle invasive bladder cancer.

[0016] Another embodiment of the invention is a pharmaceutical composition of the one or more strain(s) of Mycobacterium described above and a pharmaceutically acceptable carrier. This pharmaceutical composition may be combined with at least one or more compounds enhancing immunogenicity described above.

[0017] Another embodiment of the invention is a method of vaccinating a subject against TB comprising administering to the subject and effective amount of the one or more strain(s) of Mycobacterium described above and a pharmaceutically acceptable carrier. This method of vaccination may also include one or more compounds enhancing immunogenicity described above.

[0018] Another embodiment of the invention is a method of treating or preventing cancer in a subject comprising administering to the subject an effective amount of the one or more strain(s) of Mycobacterium described above and a pharmaceutically acceptable carrier. This method of treating or preventing cancer may also include one or more compounds enhancing immunogenicity described above.

[0019]

BRIEF DESCRIPTION OF THE DRAWINGS

[0020] Figure 1A-1D illustrates the c-di-AMP production by A£ tuberculosis in the in vitro broth culture. Mycobacterium tuberculosis stain CDC155I was grown in Middle Brook 7H9 broth supplemented with 10% OADC, 0.5% glycerol and 0.05% Tween 80 and at various stages of growth, nucleotides were extracted and analyzed for the presence of c-di- AMP. LC-MS-MRM chromatograms of (a) intracellular (intra-bacterial) and (b) secreted (culture supernatant) c-di-AMP detected from M. tuberculosis culture at an O.D. (A«xmm) of 1. (c) intra-bacterial levels of c-di-AMP extracted from 2x10^s bacilli at the indicated culture O.D. Data is Mean plus/minus SD of triplicate samples, (d) intre-macropbage (per 6xl0^fi J774 cells) levels of M. tuberculosis secreted c-di-AMP at 24hr after infection with an MOI of 1:20. Data is Mean plus/minus SD of triplicate samples.

[0021] Figure 2A-2D illustrates generation and confirmation of M. tuberculosis over expression, (a) The disA gene of M. tuberculosis, MT3692, was PCR-amplified from M. tuberculosis CDC1551 genomic DNA using gene-specific primers. The amplicons were cloned into the mycobacterial expression vector pSD5-hsp60 at the Nde I and Mlu I restriction sites, (b) The resulting construct pSD5-hsp60-MT3692 was sequenced and used to transform M tuberculosis CDC1551 and recombinant clones were selected against

Kanamycin (25ug ml). Colony PCR using Kanamycin gene specific primers confirmed the presence of recombinant plasmid in the Mtb-OE strain, (c) Table depicting the RNAseq. result of Mtb-CDC151 and the Mtb-OE stains for the gene MT3692 indicating approximately 95 fold over-expression of MT3692 in Mtb-OE in comparison to Mtb-CDC1551. For RNA sequencing, total RNA were extracted from M, tuberculosis cultures at an O ⁾, of 1 , followed by rRNA depletion and sequencing using Applied Biosystems SOLID™ Titak RNA-Seq Kit protocol on a AB 5500x1 SOLID sequencer, (d) Comparison of the intra-bacterial levels of c- di-AMP extracted from 2x10* cells of Mtb-CDC155I and Mtb-OE at culture O.D. of 1. Data is Mean plus/minus SD of triplicate samples; ***, < .001 by Student's t-test (2-taiIed).

[0022] Figure 3A-3C illustrates transposon insertion mutant of Mycobacterium tuberculosis CDC 15 1 for MT3692 gene is unable to produce c-di-AMP. Mycobacterium tuberculosis strain CDC1551 and Mtb-_ftj_4-K0 (JHU-3586) were grown in Middle Brook 7H9 broth supplemented with 10% OADC, 0.5% glycerol and 0.05% Tween 80 and nucleotides were extracted from bacterial pellet at culture CP. of 1. LC-MS- RM chromatograms of intracellular c-di-AMP extracted from (a) Mtb-CDC1551 and (b) Mtb- disA-KO. (c) Comparison of the intra-bacterial levels of c-di-AMP extracted from 2 x 10^s cells of Mtb-CDC1551 and Mtb- disA-KO at culture O.D. of 1 by LC-MS-MRM confirms that Mtb- disA-KO stain is devoid of c-di-AMP production.

[0023] Figure 4A-4D illustrates generation and confirmation of M tubercuIosis-CDC 1551 MT3692 complemented strain (Mtb-COMP), (a) Organization of radA-disA operon in genome of M. tuberculosis CDC1551. (b) The whole operon of rad4-disA including the upstream promoter region was PCR-amplified using M. tuberculosis CDC1 51 genomic DNA and primers OPE-MT3692(F) and OPE-MT3692(R) and cloned into an integrative vector, pMH941-Hyg, at Xbal- restriction site, (c) The resulting construct, pMH94Hyg- MT3692 was used to transform the Mtb-disA-KO strain (JHU-3586). Candidate Hyg^R colonies were selected and genomic DNA from the Mtb-COMP clones were used for PCR based confirmation using Hygromycin gene specific primers, (d) Comparison of the intra- bacterial levels of c-di-AMP extracted from 2 x 10⁸ cells of Mb-disA-KO and Mtb-COMP at culture O.D. of 1 by LC-MS-MRM confirms the reconstitution of c-di-AMP production in the Mtb-COMP strain.

[0024] Figure. 5 illustrates Interferon Regulatory Factor (IRF) pathway activation following infection with various tuberculosis strains with varied levels of c-di-AMP production. TOP 1 -Dual™ cells (InvivoGen) were grown as per the supplier's

recommendations. Twenty four hours after infection of PMA activated THP-DuaP* cells with a pre-calibrated MOI of 1:10, culture supernatants were separated and used for measurement of IRF pathway activation by Quanti-Luc™ assay. Data are mean plus/minus SE at the least three experiments (n=3); * p<0.05,***,p 0.00l by Student's test (2-tailed).

[0025] Figure 6A-6F illustrates increased induction of pro-inflammatory cytokines following infection with the c-di-AMP over-expressing tuberculosis strain. Levels of (a,b) IL-Ια, (c,d) IL-6 and (e,f) TNF-a in culture media at 24 h post-infection from BMDM and BMDC cells infected with various M. tuberculosis strains at an MOI of 1 : 10. Data are mean plus/minus SE of at the least three experiments (n=3). *, p<0.05 and **, pO.Ol by Student's t-test (2-tailed).

(0026] Figure 7 illustrates in vitro growth pattern of M. tuberculosis strains possessing different c-di-AMP production levels. Mycobacterium tuberculosis strains were grown in Middle Brook 7H9 broth supplemented with 10% OA C, 0.5% glycerol and 0.05% Tween 80 for 20 days. At the indicated time points after inoculation, samples were collected and absorbance (Αώ») were measured by spectrophotometer. Comparable growth was observed amongst all the M. tuberculosis strains. Data are mean of triplicate samples. Error bars are overlapping and not shown for clarity of the line diagram.

[0027] Figure 8A-8B illustrates increased phosphorylation of TBKl in macrophage following infection with the Mtb-OE strain, (a) Fluorescence microcopy merged (Blue + Green channel) images of J774 cells, fixed after 6 hr of infection with various M. tuberculosis strains and stained with anti-pTBKl antibody, Nuclei-Blue PAPI), pTBKl-Green (AF488). (b) Quantitative analysis of pTB l positive staining of the infected macrophage cells revealed significantly higher percentage of cell exhibiting increased staining for pTBKl in case of Mtb-OE infection in comparison to infection with other Mtb-strains. Box plot depicting Mean (+), Median (-) with quartiles (box margins) and ranges (bars) (n=6). *, p<0.5 and ***, p<0.001 by Student's t-test (2-tailed).

[00281 Figure 9A-9D illustrates knock down of DDX41 in macrophage leads to reduced induction of type I IFN and TNF-oc response, (a) Western blot analysis of DDX41 and GADPH (loading control) of DDX41 Knock down (KD) and control (WT) RAW-Blue™ ISG ceils and densitometry analysis of the western blots showing approximately 30% reduced DDX41 protein level in the KD cells. Data are mean from duplicate experiments, (b) As an indicator of IRF induction, levels of SEAP in the supernatant of DDX41 Knock down (KD) and control (WT) RAW-Blue™ ISG cells at 18 hr after infection with various M, tuberculosis strains were measured by a spectrophotometer following Quanti-Blue™ assay, (c) Levels of IFN-β and (d) TNF-a in culture media of DDX4I Knock down (KD) and control (WT) RAW-Blue™ ISG cells at 18 hr after infection with various M. tuberculosis strains atMOI of 1 :5 were measured by ELISA. Data are mean plus/minus SE of at the least three experiments (n=3). ·*, p<0.0.5 and ***, p<0.001 by Student's t-test (2-tailed). (0029J Figure 1 OA- 1 OH illustrates modulation of host cytokine response and intracellular growth of M. tuberculosis by c-di-AMP. (a) Levels of IFN-β in culture media at 24h post- infection from resting and (b) IFN-pY LPS activated J774.1 cells infected with various Mtb- strains at an MOI of 1 :20. (c) Levels of TNF-a in culture media at indicated time points from resting and (d) IFN-p/ LPS activated J774.1 cells infected with various Mtb-strains at an MOI of 1 :20. (e) Levels of IFN-β in culture media at 24h post-infection from BMD and (f) BMDC ceils infected with various Mtb-strains at an MOI of 1 : 10. ELISA Data are mean ± SE of at the least three experiments (n = 3). *, p < 0.05; **, p < 0.01 and ***, p < 0.001 by One-way ANOVA with Tuke 's post test, (g) IFN-β mRNA were assessed by qRT-PCR in BMDCs infected with various Mtb-strains at 24h post-infection; data are mean ± SD (n = 3) and representative of two experiments. **, p < 0.01 and ***, p < 0.001 by One-way ANOVA with Tukey's post test, (h) Growth kinetics of various Mtb-strains in resting and (i) IFN-D/ LPS activated J774.1 ceils. Data are Mean CFUs ± SD at each time point (n = 3) and representative of two experiments. Bar diagrams (right panels in h and i) represent Mean CPUs ± SD at Day 4. *, p < 0.05 and ***·, p < 0.001 by Student's t-test (2-tailed).

10030] Figure 1 lA-11C illustrates c-di-AMP produced by M. tuberculosis induces autophagy in macrophage cells, (a) Fluorescence confocal images of J774.1 cells, fixed after 6 hr of infection. with various M. tuberculosis strains and stained with anti-LC3 antibody; Nuclei-Blue (DAPI), LC3b-Green (AF488). Scale bars depicts 20 μ^ηι for 40X images and 10 μηι for 100X images, (b) Quantitative analysis of LC3 positive J774.1 cells showing puncta formation, Only those cells were considered as positive and included for quantification, which exhibited formation of large LC3 aggregates occupying area > Ιμπι, Percentage of LC3-II positive cells were calculated and data are depicted by box plot indicating Mean (+), Median (-) with quartiles (box margins) and ranges (bars) (n = 9). *, p < 0.05; **, p < 0.01 and ***, p < 0.001 by One-way ANOVA with Tukey's post test, (c) Western blot analysis of LC3-I and LC3-I1 and GAPDH (loading control) of J774.1 cells at 6 hr after infection along with bar diagram depicting densitometric ratios of normalized LC3-H/LC3-I levels. Data are mean ± SD (n ~ 2) from two experiments *, p < 0.05 by Student's t-test (2-tailed).

[0031] Figure 12A-12H illustrates attenuation of virulence and pathogenicity in c-di- AMP over-producing M. tuberculosis strain, (a) Survival of mice (n = 10) following infection with various Mtb-strains. ***, p < 0.001 by Log-rank (Mantel-Cox) test, (b) Growth kinetics of various . tuberculosis-strains in mouse lungs and (c) spleen after aerosol infection. Data are mean ± SE (n = 4). *, p < 0.05; **, p < 0.01 and ***, p < 0.001 by Two-way ANOVA with Bonferroni post-test, (d) Gross and (e) histo-pathologica⁾ features of lungs and spleen of mouse infected with various M. tuberculosis-strains. Scale bar is 100 μπι. (f) Levels of IFN- β, (g) TNF -a and (h) IFN-p in the serum of mice infected with M. tuberculosis-strains possessing varied ability to produce c-dt-AMP. Data are mean ± SE (n = 4). *, p < 0.05; **, p < 0.01 and * **, p < 0.001 by Student's t-test (2-tailed).

[0032] Figure 13A-13H illustrates contribution of STING and cytosolic DNA receptor cGAS to c-di-AMP mediated activation of IFN-p during M. tuberculosis infection, (a, c) IRF pathway activation as measured by luciferase reporter assay and (b, d) IFN-β levels in the 18h post-infection (MOI = 1 ·5) and post-stimulation culture supernatants of mouse RAW264.7 derived STING ablated [STTNG-KO] and control [WT] macrophage IRF reporter cells, (e) IFN-p induction in BMDMs and (fj BMDCs from control [WT] and cGAS ablated [cGAS- O] mouse following infection (MOI = 1 :10) with various Mycobacterium strains, (g) c-di- ' AMP concentration dependent induction of IFN-β in mouse BMDMs. Data are mean * SB of at the least three experiments (n = 4 in a, b; n = 3 in c, d, e, f, g).*, p < 0.05; **, p < 0.01 and ***, p < 0.001 by Student's t-test (2-tailed). (h) Levels ofIFN-β mRNA were determined by real-time RT-PCR in BMDCs derived from wild type cGAS sufficient [WT] and cGAS ablated [cGAS-KO] mouse following infection (MOI = 1:10) with various Mycobacterium strains. The lFN-β mRNA expression levels were normalized to -actin expression and are represented relative to those of untreated cells. Data are mean -fc SD (n = 3) and is representative of two experiments. *, p < 0.05; ** p < 0.01 and ***, p < 0.001 by Student's t- test (2-tailed).

[0033] Figure 14 illustrates plasmids and Mycobacterium used in the invention.

[0034] Figure 15A-15B illustrates aj Mice experiments with a strain of BGC including an expression vector encoding a diadenylate cyclase protein (rBOG-di&A) and b) Graph of CFU one day post infection.

[0035] Figure 16 illustrates the gross pathology of organs 18 weeks post infection from mice described in Figure 15.

[0036] Figure 17A- 17B illustrates a) lung and b) spleen CFU 18 weeks post infection from mice described in Figure 15. [0037] Figure 18A-18B illustrates the a)prophyIactic potential of BCG strain including a DNA expression vector encoding disA (rBCA-disA) in guinea pigs and b) CFU one day post infection.

[0038] Figure 19 illustrates the gross pathology and CFU of lungs 14 weeks post- . infection of the guinea pigs described in Figure 18.

[0039] Figure 20 illustrates the gross pathology and CFU of spleen 14 weeks postinfection of the guinea pigs described in Figure 18.

[0040] Figure 21 illustrates the gross pathology of lungs 18 weeks post-infection of the guinea pigs described in Figure 18.

[0041] Figure 22 illustrates the gross pathology of spleen 18 weeks post-infection of the guinea pigs described in Figure 18. '

[0042] Figure 23 illustrates the graphs of lung and spleen infection of the guinea pigs described in Figure 18.

DETAILED DESCRIPTION OP THE INVENTION

[0043] As. shown in Fig. 1, M. tuberculosis produced and secreted c-di-AMP. The amount of c-di-AMP was quantified in a 7H9 broth culture and within the bacteria

(intracellular). Intracellular c-di-AMP levels were observed to increase during late-log and stationary phases of growth of M. tuberculosis compared to early log phase growth. After 24 hours of infection of J774 mouse macrophage cells with M tuberculosis, the c-di-AMP produced by the bacteria was detected in the macrophage cytosol of die J774 cells.

[0044] Strains of A£ tuberculosis, producing different amounts of c-di-AMP, were formed and then used in studies of the present invention. As illustrated in Fig.2, a recombinant M. tuberculosis strain Mtb-OE (OE means "over expression" of c-di-AMP) was formed having over 95-fold expression of an endogenous di-adenylate cyclase gene, disA, and a resultant increase in the production of c-di-AMP by -20 fold when compared to the M. tuberculosis CDC 1551 a wild type (WT) strain of M. tuberculosis. As described in SUPP FIG. 3, a recombinant M. tuberculosis strain Mtb-disA- O (KO means "Knock Out" of the disA gene) was produced with a transposon insertion disrupting the di-adenylate cyclase domain of disA making the strain substantially free of c-di-AMP. c-di-AMP is produced by a single di-adenylate cyclase in M. tuberculosis so knocking out this gene knocks further knocks out c-di-AMP production. As shown in Fig. 4, a strain Mtb-COMP was formed by taking the Mtb-disA-KO strain and transforming it with an expression vector with an endogenous disA gene and native promoter The addition of the expression vector reconstituted c-di-AMP production in Mtb-disA-KO.

[0045] As shown in Fig. 10_» J774.1 mouse macrophage cells were infected with these M. tuberculosis strains (Mtb-CDC1551, Mtb-disA-KO, Mtb-COMP, and Mtb-OE) expressing different amounts of c-di-AMP in vitro. After different incubation times, the amount of IFN-β produced by the J774.1 cells were measured. As shown in Fig. 10, infection with the Mtb- disA-KO strain resulted in a significant reduction in IFN-β induction by J774.1 cells compared to infection with the Mtb-CDC1551. Conversely, infection with the Mtb-OE strain resulted in an enhanced induction of IF -β by both resting and activated J774.1 cells.

Notably, Mtb-OE infected cells also secreted significantly higher levels of TNF-a compared to the Mtb-WT infected cells (or Mtb-CDC1551), whereas Mtb-disA-KO infected cells produced lower TNF-a levels compared to other groups (Fig. lOc, d). As shown in SUPP FIG. 5, the patterns of Interferon Regulatory Factor (IRF) pathway activation in THPl- human monocyte cells was analyzed and IFN-β responses in mouse primary bone marrow derived macrophages (BMDM) and dendritic cells (BMDQ (Fig. 10e, f) were comparable. However, the mouse BMDCs are a comparatively better IFN-β producer than BMDMs in response to M. tuberculosis infection. Induction of IFN-β was further confirmed by real time RT-PCR of the BMDC cells infected with the various M. tuberculosis strains (Fig. lOg). We also observed induction of significantly higher levels of proinflammatory cytokines including IL-1 a, IL-6 and TNF-a by both BMDMs and BMDCs following infection with the c-di-AMP over-expressing M. tuberculosis strain Mtb-OE (Fig. 6). These observations suggest that perturbation of c-di-AMP levels in M. tuberculosis not only influences the CSP mediated Type I IFN response but also plays a critical role in modulating the proinflammatory cytokine signature of the infected cells.

[0046] Taking into account the ambiguous role of the Type I IFN response in host control of TB, the growth patterns of these M. tuberculosis strains in resting and IFN-p LPS activated J774.1 cells were monitored. While all M. tuberculosis WT and recombinant strains exhibited identical growth rates in 7H9 broth culture (Fig. 7), the Mtb-OE strain over expressing c-di- AMP exhibited significantly diminished intracellular growth compared with the other M. tuberculosis strains (Fig. lOh, i). Growth attenuation of the knock out strain Mtb-disA-KO which is c-di-AMP deficient strain was not noticed. These observations reveal that over- expression of c-di-AMP by tuberculosis results in significant attenuation of the intracellular growth of the Mtb-OE strain.

(0047] Next, we investigated whether enhanced macrophage autophagy might account for the attenuation of the c-di-AMP over-expressing M. tuberculosis strain Mtb-OE by examining the auto-phagosome membrane specific marker LC3 in M tuberculosis infected J774.1 cells. Fluorescence confocal imaging demonstrated a considerably higher percentage of cells (-15%) exhibiting LC3 puncta formation in the case of the over expression c-di-AMP strain Mtb-OE infection compared to the wild type strata Mtb-CDC1551 (-10%) and the knock out strain Mtb-disA-KO which is c-di-AMP deficient (-6%) (Fig. 11 a, b). In addition, Western blot analysis of endogenous LC3 revealed an increase in conversion of LC3-I to LC3-II in the Mtb-OE infected cells, indicating hyper-activation of autophagy (Fig.2c). We also observed a considerably higher percentage of cells exhibiting pTBKl positivity suggesting activation oflRF pathway in the Mtb-OE infected J774.1 cells (Fig. 8). These observations strongly suggest that hyper-induction of autophagy by macrophages may be one of the contributing factors that restricts the intracellular growth of Mtb-OE strain.

[0048] The virulence and pathogenicity of the M. tuberculosis strains in mouse aerosol infection models were examined. Remarkably, compared to WT infection using strain Mtb- CDC1551 (median time to death [MTD] of 150 days), a significant increase in the survival of Mtb-OE infected mice (MTD 321 days) was observed. In contrast, the knock out strain Mtb- disA-KO which is c-di-AMP deficient showed reduced survrval with an MTD of 77 days (Fig. 12a). Concomitantly, the Mtb-OE strain also exhibited growth attenuation as evidenced by significantly reduced lung and spleen bacillary ads (Fig. 12b, c). Gross and histo- pathological findings of mouse lungs and spleens correlated well with the bacterial organ burden observations (Pig. I2d, e). The lungs of Mtb-OE infected-mice showed significantly fewer and smaller tubercle-like lesions compared to other groups. Concordantly, while Mtb- CDC155I, Mtb disA-KO, and Mtb-COMP strain-infected mice exhibited considerable splenomegaly, spleens of the Mtb-OE infected mice appeared normal in size (Fig. 12d).

Altogether, these observations clearly demonstrate attenuation of virulence in the c-di-AMP over-expressing M. tuberculosis strain. [0049] The mouse serum cytokine levels between these groups at an early stage of disease of 2 weeks post-infection were compared. Consistent with the in vitro studies in mouse and human ceils, we observed increased IFN-β levels in the serum of Mtb-OE infected mice compared to the Mtb-CDC1551 and Mtb-disA-KO group (Fig. I2f). In addition, the Mtb-OE group exhibited significantly higher serum levels of TNF-a (Fig. 12g). Since Type I IFN (IFN-β) is known to counter-regulate Type IT IFN (IFN-β) responses, we measured IFN- β levels in the serum of infected mice (Fig. 12h). A strong inverse relationship between IFN- β and IF Py in these mice corresponds to the ability of the M. tuberculosis-strains to produce c-di-AMP.

[0050] These studies revealed bacterial c-di-AMP levels are strongly associated with the immunopathological outcome of bacterial infection, including M. tuberculosis, in mice. Next, the host cytosolic sensors that may detect M. tuberculosts^emed c-di-AMP starting with helicase DDX41, a cytosolic DNA, and CDN receptor that signals via STING were examined. A shRNA-mediated knocked down of DDX41 using RAW- BlueTM ISG cells (InvivoGen) that allow colorimetric measurement of the induction of the IRF pathway was performed. Knockdown of DDX41 caused a significant defect in activation of the ERF pathway and reduced IFN-β induction following infection with all the M. tuberculosis strains (Fig.9a, b, c). We also observed a significantly reduced TNF-a production by the DDX41 knock-down cells (Fig. 9d). These results suggest that DDX41 is a key pattern recognition receptor for both DNA and c-di-AMP, and that DDX41 regulates the induction of Type I IFNs as well as TNF-a following M. tuberculosis infection.

[0051] The contribution of STING to the c-di-AMP-mediated IFN-β response during M. tuberculosis nfection was investigated. A partial knock-down of STING in human ΊΉΡ1 cells showed considerably lower IFN-β induction than control cells (Fig. 10). Moreover, all M. tuberculosis strains failed to activate the IRF pathway or induce IFN-β in mouse RAW 264.7 macrophage IRF reporter cells lacking STING (STING-KO) (Fig. 13a, b, c, d).

However, LPS, which stimulates Type I IFN through STING-independent pathways, induced elevated IFN-β response even in STING-KO cells (Fig. 13a, b). These results confirm that, in addition to its role in bacterial DNA mediated responses, STING is an essential component for c-di-AMP-mediated activation of the IRF pathway during M. tuberculosis infection. Furthermore, infection of macrophages with M. bovis bacille Calraette-Guerin (BCG), which is known to lack the Esx-I secretion system, also showed activation of the IRF pathway at levels 20-60% of those seen following infection with either the Mtb-CDCl 551 or the Erdman strain, a WT M. tuberculosis strain considered to be highly virulent (Fig. 13a, b).

Importantly, the c-di-AMP over-expressing , bovis BCG strain (BCG-OE) produced a significantly higher IRF and IFN-β response than M. bovis BCG itself, thus strongly suggesting that bacterial-derived c-di-AMP gains access to the host cell cytosol despite the absence of an Esx-1 secretion system (Fig. 13a, b). These experiments indicate that, while contributory to overall type I IFN response, Esx-1 may not be essential for c-di-AMP- triggered IRF pathway activation. However, further studies with ESX-1 deleted M.

tuberculosis strains may provide lirect evidence for contribution of ESX-1 secretion system in c-di-AMP mediated responses during M. tuberculosis infection.

[0052] Next, the role of cGAS in the detection of bacterial c-di-AMP was examined. Primary BMDMs (Fig. 13e) and BMDCs (Fig.4f) from WT and cGAS-KO mice22 were infected with these mycobacterial strains and then IFN-β protein levels were measured. While loss of cGAS resulted in a considerably reduced IFN-β response compared to cells with intact cGAS (WT), all c-di-AMP overproducing strains continued to show significantly higher induction of IFN-β in cGAS-KO cells compared to their respective WT mycobacterial strains (Fig. 13e, f). Further, both WT and cGAS-KO BMDMs produced comparable levels of IFN-β following stimulation with synthetic c-di-AMP (Fig. 13g). Real time RT-PCR for IF -β in BMDCs further confirmed these results (Fig. 13h). These experiments show that while c-di-AMP is a key ligand for IFN-β induction irrespective of cGAS, a significant part of the overall IFN-β response during M tuberculosis infection is cGAS dependent and hence is probably due to bacterial DNA.

[0053] The data thus revealed the involvement of c-di-AMP as an tuberculosis Pathogen Associated Molecular Pathway (PAMP) that triggers host cell TFN-β secretion and autophagy. Our findings, which employed multiple bacterial strains (including the wild type M. tuberculosis CDC1551 and Erdman strains, and ML bovis BCG) were each modified to overexpress c-di-AMP and a variety of host phagocytic cells including those defective in important mediators of the CSP (STING, DDX41, and cGAS), consistently demonstrated that c-di-AMP, not bacterial DNA alone, is a key mediator of Type 1 IFN responses.

Supplementary Table 1 lists major differences in our methods compared with those of earlier studies and reveals that strain, host cell, and methodological differences may have allowed the importance of c-di-AMP to have been overlooked in earlier studies. The studies have . shown that c-di-AMP enhances the induction of Type I IFN in subjects as well as several pro-inflammatory cytokines including ILl-ct, TNF-a and IL-6 that are believed to play protective roles during bacterial infections such as a M. tuberculosis infection. The data illustrates that resistance to tuberculosis (TB) requires CSP-mediated detection of c-di-AMP produced by M, tuberculosis and that levels of c-di-AMP modulate the fate of infection. A di- adenylate cyclase (disA or dacAf over-expressing M tuberculosis strain was formed mat secretes excess c-di-AMP and activates the interferon regulatory factor (IRF) pathway with enhanced levels of IFN-β, elicits increased macrophage autophagy, and exhibits significant attenuation in mice. c-di-AMP-medtated IFN-β induction during M. tuberculosis infection was shown to require stimulator of interferon genes (STlNG)⁵-signaling. c-di-AMP induction of IFN-β is independent of the cytosoHc nucleic acid receptor cycUc-GMP-AMP (cGAMP) synthase (cGAS), but cGAS nevertheless contributes substantially to the overall IFN-β response to M. tuberculosis infection. The present invention demonstrates c-di-AMP to be a key mycobacterial pathogen associated molecular pattern (PAMP) driving host Type I IFN responses and autophagy. Modulating the levels of c-di-AMP in a subject will enhance the subject's immune response and may be used to treat disease including immune-deficient disease such as HTV and bacterial infections including TB.

[0054] Hence, in this study we generated a recombinant BCG that over-expresses diadenytate cyclase (disA) oiM. tuberculosis (Rv3586) and tested the prophylactic potential of rBCG-disA as a vaccine in mouse and guinea pig model of aerosol tuberculosis infection and also tested its ability to induce Type I IFN response. BCG strains modified to over-express c-di-AMP exhibited marked improvement in protective immunity against tuberculosis as evidenced by marked reduction in lung and spleen bacillary load and reduced pathology in guinea pig and mouse models of infection. In addition, in vitro studies in RAW cells revealed that, a c-di-AMP-over-expressing BCG strain (rBCG-disA) produced a significantly higher IRF activation and IFN-β response than BCG itself, suggesting that bacteria-derived c-di-AMP gains access to the host cell cytosol despite the absence of an ESX-1 protein secretion system in the BCG strain and can potentiate the ability of BCG to induce higher IFN-β response. [0055] Methods In this study we generated a recombinant BCG that over-expresses diadenylate cyclase (disA) ofM. tuberculosis (Rv3586) and tested the prophylactic potential of rBCG-disA as a vaccine in mouse and guinea pig model of aerosol M tuberculosis infection and also tested its ability to induce Type I IFN response and dependence on STING (Stimulator of Interferon Genes) and cGAS (cyclic GAMP Synthase) signaling axis..

[0056] Results BCG strains modified to over-express c-di-AMP exhibited marked improvement in protective immunity against tuberculosis as evidenced by marked reduction in lung and spleen bacillary load and reduced pathology. In addition, fn vitro studies in RAW cells revealed that, a c-di-AMP-over-expressing BCG strain (rBCG-disA) produced a significantly higher IRF activation and IFN-β response than BCG itself in a STING dependent and cGAS independent manner, suggesting that bacteria-derived c-di-AMP gains access to the host cell cytosol despite the absence of an ESX-1 protein secretion system in the BCG strain and can potentiate the ability of BCG to induce higher IFN-β response.

[0057] We hypothesized that over-production of c-di-AMP by BCG may offer a multi- pronged approach to tap the adjuvant potential of c-di-AMP to improve the protective potential of BCG via (i) enhancing the type I IFN and other pro-inflammatory cytokine responses compared to BCG; (ii) enhancing the intrinsic ability of BCG to cause DC maturation; (iii) enhancing over-all antigen presentation following BCG vaccination via induction of higher levels of autophagy and induction of co-stimulatory molecules by this rBCG. The method disclosed in the present invention depends on the over-production of c- di-AMP by rBCG-disAOE. The present invention thus, provides a novel way to improve the existing BCG vaccine intrinsically without the need of exogenous addition of cytokines or use of synthetic chemicals or nucleotide molecules.

[0058] The present invention provides an improved method of immunization against tuberculosis using recombinant BCG-disAOE (rBCG-disAOE). The method disclosed in the present invention depends on the over-production of c-di-AMP by rBCG-disAOE.

Mycobacterium bovis BCG Pasteur strain over expressing disA (JRv3S8S gene of

Mycobacterium tuberculosis under the transcriptional control of a strong mycobacterial promoter hsp60 using mycobacterial vectors described (DasGupta, Jain et al. 1998; Dhar, Rao et al. 2000; Jain, Dey et al. 2008). In the present invention, the protective efficacy of rBCG was assessed in mouse and.a highly susceptible guinea pig model against M. tuberculosis challenge by the aerosol route as described before (Jain, Dey et al.2008; Dey, Jain et ai.2011).

[0059] Immunization of mouse with rBCG resulted in a significantly enhanced protection characterized by a marked reduction in bacilJary load in lungs (1.162 logio) and spleen (0.72 logio) compared to sham-immunized mice at 10 weeks post-infection. However, at this time point differences in CFU were not significantly different from BCG. Further at 18 weeks pos- infection, the extent of reduction in lung CFU in case of rBCG-disAOE immunization was markedly greater when compared to sham (by 0.35 logio) and BCG (by 0.49 logio), immunized animals signifying greater protection against pulmonary disease.

[0060] Most significant effect of rBCG immunization on disease control, both in terms of reduction in bacillar load and pathology was evident in guinea pig model of M. tuberculosis infection. Wherein, immunization with b m BCG as well as with rBCG-disAOE resulted in a significant reduction in lung and spleen bacillary load, when compared to the saline treated animals at 14 weeks post infection along with marked improvement in disease pathology as evidenced by reduced organ weight and pathology scores. However, the extent of reduction in bacillary burden in case of rBCG-disAOE immunization was markedly greater (by 0.37 logio in lung and 1.6 logio in spleen), when compared to BCG immunized animals. Further, at 18 weeks post-infection along with a markedly reduced disease pathology, rBCG immunized animals exhibited a markedly reduced lung (by 2.49 logio) and spleen (by 4.68 logio) bacillary burden when compared to sham immunized animals. Most importantly. rBCG treated animals showed a marked improvement when compared to BCG treated animals both in terms of lung and spleen bacillary burden (by 1.9 logio and 2.54 logio, respectively). [See attached Figures]

EXAMPLES

[0061] Bacterial strains, plasmids, cell lines and animals. In this study we used Escherichia coli strain DH5a, M tuberculosis CDC1551, M. tuberculosis Erdman, M. hovis bacillus Calmette-Guerin (BCG). Figure 14 lists all the Mycobacterium strains and plasmids used in this study. Details on the transposon insertion mutant of M. tuberculosis for MTB692 {M. t berculosis-mutaat JHU-3586; v3586) used in this study is available on the TARGET website of the Johns Hopkins University. Plasmid pSD5-hsp60 (mycobacteria-..-', coli shuttle vector for protein expression in M. tuberculosis from the strong mycobacterial promoter, hsp60) was used for expression. Plasmid pMH94Hyg was used for complementation. Both E coli and mycobacterial strains were grown from frozen glycerol stocks stored at -70 °C. Murine macrophage cells J774.1, RAW 264.7-derived macrophages such as RAW-Blue ISG, RAW-Lucia ISG, RAW-Lucia TSG-KO-STI G (Sting knockout cells), human monocyte THPl-Dual, THPl-Blu TSG-KD-STING cells (all from InvivoGen) and primary BMDMs and BMDCs from C57BL/6J and cGAS- O mouse were used for in vitro experiments. Ail cell lines are free of mycoplasma contamination. Female mouse strains BALB/c and C57BL 6J (Jackson laboratories), age 6-7 weeks, were used for comparative studies of bacterial virulence, pathogenicity and time to death. The experiments were approved by the

Institutional Animal Care and Use Committees (lACUCs) of Johns Hopkins University.

[0062] Reagents. J774.1 cells were cultured in RPMI-GIutaMAX (Life Technologies) with 10% (vol/vol) heat-inactivated FBS (Life technologies). Variants of RAW264.7 and THP-l cells were cultured as per the suppliers protocol (InvivoGen) in DMEM and RPMI- GlutaMAX, respectively (Life Technologies) with 10% heat-inactivated FBS. The following antibodies were used: antibody to DDX41 (anti-DDX4I; G14; Santa Cruz Biotechnology ϊηο. 1:500); anti-LC3A/B (D3U4C, XP; Cell Signaling Technologies, 1 : 1,000); anti-STING (D2P2F; Cell Signaling Technologies, 1:1,000); anti-pTBKl (Serl72, P52C2; Cell Signaling Technologies 1:1,000); anti-GAPDH (14C10; Cell Signaling Technologies, 1:2,000).

Secondary antibody anti-rabbit conjugated to fluorochrome Alexa Fluor 488, DAP1 (Life Technologies), c-di-AMP (BIOLOGLife Science Institute), c-di-UMP, puromycin, 2eocin, blasticidin, Quanti-BIue, Quanti-Luc (InvivoGen), hygromycin (Roche) and kanamycin (Sigma-AIdrich).

[0063] Extraction of nucleotides from M. tuberculosis and detection and quantitation of c-di-AMP by LC-MS/MS/MRM. Nucleotide extraction for LC-MS/MS were carried out as described42. Briefly, M. tuberculosis was grown to mid-log phase and harvested by quick centrirugation followed by resuspension in extraction buffer containing acetonitrile and methanol and water (2:2.1) and cXMP as an internal technical control. After a 15-min incubation and subsequent boiling at 100 ^CC for 10 min, the mixture was cooled down and extracted after quick centrifugation. Extraction was repeated twice as described above.

Pooled samples were vacuum dried and resuspended in distilled water followed by detection and quantitation by LC-MS MS MRM. Briefly, the chromatographic separation was performed on a Series 200 HPLC system (Perkin Elmer Instruments) and the analyte detection was performed on an API 3000 triple quadrupole mass spectrometer equipped with an electrospray ionization (ESI) source (Applied Biosystems Inc.) using RM analysis in positive ionization mode. The following SRM transitions using a dwell_^time of 40 ms were detected: cXMP: +347.1/153 (quantifier), +341.7/136 (identifier) and c-di-AMPr

+659.1/330.2 (quantifier) and +659/524 (identifier).

[0064] Extraction of nucleotides from macrophage cytoplasm and detection and quantitation of c-di-A P by LC-MS MS/M M. J774.1 cells were cultured in RP I medium with 10% heat-inactivated FBS. Infections were carried out in either resting or IF - γ- and LPS-activated J774.I cells in six-well plates in triplicate. For infection, early log- phase cultures of various Mycobacterium tuberculosis sttains were washed and diluted appropriately to predefined concentrations in antibiotic-free RPMI and were added to the J774.1 cells at a precalibrated MOI. The infection was allowed to continue for 4 h, following which extracellular bacteria were removed by washing the infected cells with DPBS thoroughly. After 24 h of infection, supernatants were removed andadherent macrophages were washed carefully with DPBS. Macrophages were lysed with the addition of 1 ml of 0.025% SDS (at this concentration of SDS, bacteria is not lysed) to each of the wells.

Released bacilli were subsequently separated by centriftigation followed by filtration through a 0.2-μηι membrane filter, and bacteria-free pooled macrophage cytoplasmic extracts were used for extraction of nucleotides and subsequent analysis by LC-MS MS as described above.

[0065] Overexpression of MT3692 iu At. tuberculosis. The disA gene of U.

tuberculosis, ΜΓ3692, was PCR-amplified from M. tuberculosis CDC1551 chromosomal DNA using gene-specific primers, pSD5hsp60.MT3692(F) and pSD5hsp60.MT3692(R). The amplicons were cloned into the Mycobacterial expression vector pSD5-hsp60 at the Ndel and Mini restriction sites. The resulting construct pSD5-hsp60-MT3692 was sequenced and subsequently used to transform M. Tuberculosis CDCI5 1 and recombinant clones were selected against kanamycin and confirmed by colony PCR using kanamycin gene-specific primers. Overexpression of Μ 3692 in the Mtb-OE strain was further confirmed by RNA sequencing of the Mtb-OE strain and measurement of c-di-AMP by LC-MS-MRM.

Overexpression of ΜΓ3692 in the M. tuberculosis Erdman and M. bovis BCG strains were carried out using the same plasm id. [0066] Construction of MT3692 complementation strain. To complement the transposes mutant for ΜΓ3692, a 279-bp DNA fragment including the coding sequence of the ΜΠ692 gene and 1,714 bp of the 5' sequence (including the upstream gene in the operon and gene's native promoter) was amplified by PCR with primers OPE-MT3692(F) and OPE- MT3692(R) and cloned into an integretion vector, pMH94Hyg, at an Xbal restriction site. The resulting construct, pMH94Hyg-MT3692, was subjected to nucleotide sequencing and subsequently used to transform the Mtb-iftivf-KO strain. Candidate Hygromycin resistant Mtb-CO P colonies were selected, confirmed by PCR using hygromycin gene-specific primers and genomic DNA as template. Mtb-COMP clones were further confirmed by measurement of c-di-AMP by LC-MS/MRM method.

[0067] Infection of mice with M. tuberculosis and assessment of bacterial load, pathology and time to death. Four strains iM. tuberculosis, Mtb-disA-KO, Mtb-COMP, Mtb-OE and Mtb-WT were used to infect 6-7-week-old female C57BL/6J mice by the aerosol route in a QIascol inhalation exposure system (Glascol) with an inoculum that implanted *-3.0 LoglO c.fi in the lungs at day I (w = 3 mice in each group). Animals from a narrow range of weight and age groups were randomly allocated for infection with different bacteria] strains. Eight mice from each group were subsequently sacrificed at 2, 4, 8 and 12 weeks after infection to determine the lung and spleen cf.u. counts (n = 4) and

histopathology and immunology studies (« = 4). Lung and spleen tissues were homogenized in their entirety in PBS and colonies were enumerated on selective 7H1 plates after 3-4 weeks of incubation at 37 °C. The number of colonies were counted and expressed as loglO cf.u. per organ. All groups were coded during the experiments. For histopathology, whole lungs were fixed in 10% buffered formalin and sections of 5 pm in thickness from formalin fixed and paraffin embedded tissues were cut onto glass slides and stained with H&E for histopathological examination. For time to death assay 6V7-week-old female BALB/c mice (n = 10 per group) were infected as described above with -3.5 loglO c.£u. of various strains of M. tuberculosis and monitored until their death due to tuberculosis. All experiments were carried out according to the guidelines of the Institutional Animal Care and Use Committees (I ACUCs) of Johns Hopkins University.

[0068] Infection of macrophages with M, tuberculosis and assay for IR activation and IFN-b production, J774.1 cells were cultured in RPMT medium with 10% heat- inactivated FBS. Infections were carried out in either resting or IFNPy-and LPS-activated J774.1 cells in 24-welI plates in triplicate. For infection, early log-phase cultures of various M. tuberculosis strains were washed and diluted appropriately to predefined concentrations in antibiotic-free RPMI and were added to the J774.1 cells at a precalibrated MOI. The infection was allowed to continue for 4 h, following which extracellular bacteria were removed by washing the infected cells with DPBS thoroughly. Serial dilutions of the bacterial suspension and macrophage lysate were plated at day '0' in order to determine an accurate bacterial count of infection and phagocytized bacterial number. For enumeration of bacterial growth, at 1, 2 and 4 d after infection cells were harvested and lysed using 0.025% SDS. Appropriate dilutions of the lysates were then inoculated onto MB7H1 ] agar plates in duplicate and incubated at 37 °C for 3 weeks. The number of colonies was counted and expressed as log 10 c.f.u. per well. Investigators were blinded for c.f.u. analysis. Macrophage culture supematants collected at the indicated time points were used for measurement of various cytokines by ELISA. For immunofluorescence and western blot detection of LC3, at 6 h after infection macrophage cells were washed thoroughly and either fixed in 4% paraformaldehyde in PBS followed by immunofluorescence staining or lysates were prepared in RTPA buffer (Cell Signaling Technologies) for western blotting. RAW-BlueTSG and RAW-Lucia ISG or RAW- Lucia ISG-KO-STING (InvivoGen) cells were derived from the murine RAW 264.7 macrophage cell line by stable integration of an interferon regulatory factor (IRF)-inducible secreted embryonic alkaline phosphatase (SEAP) and luciferase reporter constructs, respectively. These cells without prior activation were infected with various strains of M. tuberculosis with a pre-calibrated MOI of 1 :5 for 4 h. After infection, extracellular bacteria were removed by washing the infected cells with DPBS thoroughly. After 18 h incubation in fresh DMEM, supematants were collected for estimation of IRF induction by SEAP colorimetric assay using QUA TI-Blue reagent (InvivoGen) or Luminescence assay using QUANTI-Luc (InvivoGen) and for measurement of cytokines by ELISA. THPl-Dual cells (InvivoGen) were grown as per the suppliers recommendations. THPl-Dual cells were derived from the human THP-1 monocyte cell line by stable integration of two inducible reporter constructs, a new secreted luciferase reporter gene, under the control of an ISG54 (interferon-stimulated gene) minimal promoter in conjunction with five IF -stimulated response elements and a SEAP reporter gene fused to five copies of the NF-kB consensus transcriptional response element and three copies of the c-Rel binding site. As a result, THP1- Dual cells allow the simultaneous study of the NF-kB pathway, by monitoring the activity of SEAP, and the IRF pathway, by assessing the activity of Lucia in culture supernatants.

THPl-Blue ISG-KD-STING cells were generated from THPl-Blue ISG cells through knockdown of the STING gene, and they were cultured as per the supplier's

recommendations (InvivoGen). Mouse primary BMDMs and BMDCs were cultured and infected with piecalibrated MOIs as described above for immortalized cell lines.

[0069) shRNA-mediated interference. RAW Blue ISG (InvivoGen) cells were transfected with a pool of five lentiviral vectors carrying a target gene sequence for DDX41 or a control plasmid (pLKO. I) (Thermo Scientific), At 24 h after transfection, cells were selected by the addition of puromycin to the medium. For transfection Lipofectamine LTA Plus (Life Technologies) reagent was used as per the manufacturer's instructions.

Knockdown of DDX41 was confirmed by western blotting.

[0070] ELISA. ELISAs for IFN-β, IFNhr, IL- la, IL-6 and TNF-et were performed with the macrophage cell culture supernatants and serum of infected mice by using mouse cytokine-specific ELISA kits (eBtosciences, Biolegend) as per manufacturers' instructions. In vitro macrophage culture experiments were carried out in triplicate and at least thrice. Serum from four mice in each group were assayed by ELISA for cytokine levels.

(0071] Western blot analysis. For immunoblot analysis, macrophage cells at predefined time points after infection were collected and lysed in RIPA lysis buffer (Cell Signaling Technologies) containing complete protease inhibitors (Roche). LC3, STING, DDX41 and GAPDH western immunoreactivity assays of macrophage lysates were performed using anti- mouse antibodies per the antibody provider's (Cell Signaling Technology). Densitometry analyses of the western blots were carried out with GelQuant software.

[0072] Two-color immunofluorescence and confocal microscopy.

Immunofluorescence staining was carried out by serial incubation of fixed cells grown on culture slide chambers with LC3-specific antibody, (Cell Signaling Technology) followed by incubation with an isotype-specific, fluorochrome (Alexa Fluor 488)-labeled goat anti-rabbit antibody (A-l 1001; Molecular Probes). Nuclei were stained with DAPI. For imaging, we used an Olympus BX61 wiih Roper/Photometrics Coolsnap HQ fluorescence microscope and Zeiss LSM 510-meta confocal laser-scanning microscope at the Johns Hopkins University core microscopy facility. Slidebook (Intelligent Imaging), ZenLite (Zeiss) and ImageJ (public domain software available from the US National Institutes of Health) software were used for image acquisition and/or analysis. Investigators were blinded during analysis. For LC3 analysis a stringent threshold was set to define a 'puncta¹, such that only those cells that exhibited formation of large LC3 aggregates occupying an area >1 um were considered as positive. Extent of autophagy induction is thus represented by the percentage of LC3-positive cells.

[0073] Real-time RT-qPCR. Twenty four hours after infection with different strains of M. tuberculosis, RNA was extracted using the RNeasy Plus Micro Idt according to the manufacturer's protocol (Qiagen). RNA was reverse-transcribed using the iScript Reverse Transcription Supermix (Bio-Rad) containing oligo-dT and random primers. cDNA was used for real-time qPCR using 2X iQ SYBR Green Supermix and an iCycler (Bio-Rad). The primers for real-time RT-qPCR. The IFN-β mRNA expression levels were normalized to β- actin expression and fold induction was calculated by the AACT method relative to those of untreated cells.

Statistical analyses. For comparisons between groups, Student's /-test (two tailed), one-way ANOVA with Tukey's post-test and two-way ANOVA with Bonferroni post-test were used wherever appropriate. Differences were considered significant at at least P < 0.05. For statistical analysis, we used Prism 5 software (Version 5.01; GraphPad Software Inc.),

Claims

CLAIMS:

1. A pharmaceutical composition comprising a compound, salt, solvate, or stereoisomer of a synthetic c-di-AMP, and a pharmaceutically acceptable carrier.

2. A pharmaceutical composition comprising a compound, salt, solvate, or stereoisomer of a synthetic c-di-AMP, and at least one or more other compounds enhancing

immunogenicity, and a pharmaceutically acceptable carrier.

3. The pharmaceutical composition of Claim 2 wherein the compounds enhancing

immunogenicity is selected from the group consisting of mycobacterial DNA, IF , or combinations thereof.

4. A method of treating a bacterial infection in a subject comprising administering to the subject an effective amount of a compound, salt, solvate, or stereoisomer of synthetic o. di-AMP.

5. A method of treating TB in a subject comprising administering an effective amount of a compound, salt, solvate, or stereoisomer of c-di-AMP.

6. A pharmaceutical composition comprising a strain of Mycobacterium comprising an expression vector encoding a di-adenylate cyclase enzyme or functional part thereof, and a pharmaceutically acceptable carrier.

7. The pharmaceutical composition of claim 6 wherein the strain of Mycobacterium is selected from the group consisting of Mycobacterium tuberculosis or Mycobacterium bovis, or a combination thereof.

8. The phannaceutical composition of claim 7 wherein the strain of Mycobacterium is BCG.

9. The pharmaceutical composition of claim 6 wherein the expression vector is a

mycobacterial expression vector.^'

10. The pharmaceutical composition of claim 9 wherein the expression vector comprises the DNA sequence of diadenylate cyclase (disA), or a functional part thereof.

11. The pharmaceutical composition of claim 10, wherein the disA is that of M.tuberculosis (Rv3586).

12. A pharmaceutical composition of claim 6 wherein the expression, vector comprises a hsp60 promoter.

13. The method of claim 12 wherein the expression of di-adenyiate cyclase enzyme or functional part thereof is regulated by the hsp60 promoter.

1 . A pharmaceutical composition comprising a strain of Mycobacterium comprising an expression vector encoding a di-adenylate cyclase enzyme, or a functional part thereof, and at least one or more compounds enhancing immunogenicity, and a pharmaceutically acceptable carrier.

15. The pharmaceutical composition of claim 1 wherein the strain of Mycobacterium is selected from the group consisting of Mycobacterium tuberculosis, Mycobacterium bovis, or a combination thereof.

16. The pharmaceutical composition of claim 15 wherein the strain of Mycobacterium is BCG.

17. The pharmaceutical composition of claim 14 wherein the expression vector is a

mycobacterial expression vector.

IS. The pharmaceutical composition of claim 17 wherein the expression vector comprises the DNA sequence of diadenylate cyclase (disA), or a functional part thereof.

19. The pharmaceutical composition of claim 17, wherein the disA is that of M.tuberculosis (Rv3586).

20. A pharmaceutical composition of claim 14 wherein the expression vector comprises a hsp60 promoter.

21. The pharmaceutical composition of Claim 4 wherein the at least one of more compounds enhancing immunogenicity is synthetic c-di-AMP.

22. The pharmaceutical composition of Claim 14 wherein the at least one or more compounds enhancing immunogenicity is selected from the group consisting of mycobacterial DNA, IFN, or combinations thereof.

23. A method of vaccinating a subject against TB comprising administering to the subject an effective amount of a strain of Mycobacterium comprising an expression vector encoding a di-adenylate cyclase enzyme or functional part thereof and a pharmaceutically acceptable carrier.

24. The method of claim 23 wherein the strain of Mycobacterium is selected from the group consisting of Mycobacterium tuberculosis, Mycobacterium bovis, or a combination thereof.

25. The method of claim 24 wherein the strain of Mycobacterium is BCG.

26. The method of claim 23 wherein the expression vector is a mycobacterial expression vector.

27. The method of claim 26 wherein the expression vector comprises the DNA sequence of diadenylate cyclase (disA), or a functional part thereof.

28. The method of claim 27, wherein the disA is that of M.tuberculosis (Rv3586).

29. The method of claim 23 wherein the expression vector comprises a hsp60 promoter.

30. The method of claim 29 wherein the expression of di-adenylate cyclase enzyme or

functional part thereof is regulated by the hsp60 promoter.

31. A method of vaccinating a subject against TB comprising administering to the subject and effective amount of a strain of Mycobacterium over-expressing diadenylate cyclase (disA), and at least one or more other compounds enhancing immunogenicity, and a pharmaceutically acceptable carrier.

32. A method of treating or preventing cancer in a subject comprising administering to the subject an effective amount of a strain of Mycobacterium comprising an expression vector encoding a di-adenylate cyclase enzyme or a functional part thereof and a pharmaceutically acceptable carrier.

33. The method of claim 32 wherein the strain of Mycobacterium is selected from the group consisting of Mycobacterium tuberculosis, Mycobacterium bovis, or a combination thereof.

34. The method of claim 33 wherein the strain of Mycobacterium is BCG.

35. The method of claim 32 wherein the expression vector is a mycobacterial expression vector.

36. The method of claim 35 wherein the expression vector comprises the DNA sequence of diadenylate cyclase (disA), or a functional part thereof.

37. The method of claim 36, wherein the disA is that of M.tuberculosis (Rv3586).

38. The method of claim 26 wherein the expression vector comprises a hsp60 promoter.

39. The method of claim 38 wherein the expression of di-adenylate cyclase enzyme or

functional part thereof is regulated by the hsp60 promoter.

40. The method of claim 32 wherein the cancer is nonmuscle invasive bladder cancer.

41. A method of treating or preventing cancer in a subject comprising administering to the subject and effective amount of a strain of Mycobacterium over-expressing diadenylate cyclase (disA), and at least one or more other compounds enhancing immunogenicity, and a pharmaceutically acceptable carrier.

42. The method of claim 41 wherein the strain of Mycobacterium is selected from the group consisting of Mycobacterium tuberculosis, Mycobacterium bovis, or a combination thereof.

43. The pharmaceutical composition of claim 42 wherein the strain of Mycobacterium is BCG.

44. The method of claim 41 wherein the at least one or more other compounds enhancing immunogenioity is c-di-AMP.

45. The method of Claim 41 wherein the at least one or more compounds enhancing

immunogenicity is selected from the group consisting of mycobacterial DNA, IFN, or . combinations thereof,

46. The method of claim 41 wherein the expression vector is a mycobacterial expression vector. ^¾

47. The method of claim 46 wherein the expression vector comprises the DNA sequence of diadenylate cyclase (disA), or a functional part thereof.

48. The method of claim 47, wherein the disA is that of M.tubercuIosis ( v3S86).

49. The method of claim 41 wherein the expression vector comprises a hsp60 promoter.

50. The method of claim 49 wherein the expression of di-adenylate cyclase enzyme or

functional part thereof is regulated by the hsp60 promoter.

51. A strain of Mycobacterium comprising an expression vector encoding a di-adenylate cyclase enzyme.

52. The strain of claim SI, wherein the Mycobacterium is selected from the group consisting of Mycobacterium tuberculosis, Mycobacterium bovis, or a combination thereof.

53. The strain of claim 52 wherein the strain of Mycobacterium is BCG.

54. The method of claim 41 wherein the expression vector is a mycobacterial expression vector.

55. The strain of claim 54 wherein the expression vector comprises the DNA sequence of diadenylate cyclase (disA), or a functional part thereof.

56. The strain of claim 55, wherein the disA is that of M.tuberculosis (Rv3586).

57. The stain of claim 51 wherein the expression vector comprises a hsp60 promoter.

58. The strain of claim 57 wherein the expression of di-adenylate cyclase enzyme or functional part thereof is regulated by the hsp60 promoter.